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Research Article Cite This: ACS Synth. Biol. 2018, 7, 1640−1650

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Tracking of Engineered Bacteria In Vivo Using Nonstandard Amino Acid Incorporation Pichet Praveschotinunt,■,†,‡ Noémie-Manuelle Dorval Courchesne,■,†,§ Ilona den Hartog,□,†,∥,⊥ Chaochen Lu,□,†,#,∇,¶ Jessica J. Kim,⊗ Peter Q. Nguyen,† and Neel S. Joshi*,†,‡ †

Wyss Institute for Biologically Inspired Engineering, Harvard University, Boston, Massachusetts 02138, United States John A. Paulson School of Engineering and Applied Sciences, Harvard University, Cambridge, Massachusetts 02138, United States § Department of Chemical Engineering, McGill University, Montréal, Québec H3A 0C5, Canada ∥ Laboratory of Chemical Biology and Institute of Complex Molecular Systems, Department of Biomedical Engineering, Eindhoven University of Technology, 5612 AZ Eindhoven, The Netherlands ⊥ Division of Systems Biomedicine and Pharmacology, Leiden Academic Centre for Drug Research, Leiden University, 2311 EZ Leiden, The Netherlands # Dr. von Hauner Children’s Hospital, 80337 Munich, Germany ∇ Medical Center of the University of Munich, 80539 Munich, Germany ¶ Ludwig Maximilians University, 80539 Munich, Germany ⊗ Harvard College, Harvard University, Cambridge, Massachusetts 02138, United States

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ABSTRACT: The rapidly growing field of microbiome research presents a need for better methods of monitoring gut microbes in vivo with high spatial and temporal resolution. We report a method of tracking microbes in vivo within the gastrointestinal tract by programming them to incorporate nonstandard amino acids (NSAA) and labeling them via click chemistry. Using established machinery constituting an orthogonal translation system (OTS), we engineered Escherichia coli to incorporate p-azido-L-phenylalanine (pAzF) in place of the UAG (amber) stop codon. We also introduced a mutant gene encoding for a cell surface protein (CsgA) that was altered to contain an in-frame UAG codon. After pAzF incorporation and extracellular display, the engineered strains could be covalently labeled via copper-free click reaction with a Cy5 dye conjugated to the dibenzocyclooctyl (DBCO) group. We confirmed the functionality of the labeling strategy in vivo using a murine model. Labeling of the engineered strain could be observed using oral administration of the dye to mice several days after colonization of the gastrointestinal tract. This work sets the foundation for the development of in vivo tracking microbial strategies that may be compatible with noninvasive imaging modalities and are capable of longitudinal spatiotemporal monitoring of specific microbial populations. KEYWORDS: curli fibers, nonstandard amino acid, click chemistry, microbiome imaging

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microbiome from DNA and RNA sequencing of fecal and tissue samples.4−8 This approach can be noninvasive, and yields significant information about many bacterial species simultaneously, but does not give precise information about the spatiotemporal localization or density of specific microbes in the host. Other techniques, like fluorescence in situ hybridization (FISH) and immunofluorescence staining of microbes from harvested tissues, offer more spatial information.9,10 However, these methods are inherently invasive and require

tudies of interactions between resident microbes and their hosts are revealing a variety of previously unknown mechanisms by which microbes influence human physiology. The human gastrointestinal (GI) tract, which contains both the highest diversity and number of microbes in the human body, is a dynamic environment whose microbial composition can be affected by many factors, including diet, age, and immune profile.1,2 Such changes have been linked to a wide range of disease states, including inflammatory bowel disease, obesity, resistance to pathogens, diabetes, and neurodegenerative disease.1−3 These correlations have led to a need for reliable methods to monitor host−microbe interactions. A great deal has been learned about the compositional changes of the gut © 2018 American Chemical Society

Received: March 29, 2018 Published: May 23, 2018 1640

DOI: 10.1021/acssynbio.8b00135 ACS Synth. Biol. 2018, 7, 1640−1650

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ACS Synthetic Biology

Figure 1. Tracking of engineered bacteria in vivo using nonstandard amino acid incorporation. (A) Bacteria, pAzF, and imaging probe (Cy5-DBCO) are delivered orally in sequence as shown. (B) The bacteria have been engineered to express an orthogonal translation system (OTS) and a gene containing an in-frame UAG codon (csgA, orange). (C) Bacteria residing in the gastrointestinal tract incorporate pAzF and display it on their surface through the secretion and assembly of extracellular curli fibers (orange chevrons) at any point during their residency. (D) The displayed azide functional group can be targeted by an imaging probe in order to label the engineered bacterial population.

some precision using medically relevant and widely available imaging modalities. Second, it should be feasible to track the microbes longitudinally over the course of several days to months. This line of reasoning led us to a design wherein a biorthogonal click reaction is used to target an imaging probe to microbes that can stably display an appropriate click-able functional group. The imaging probe could then be delivered orally at any time point after microbial ingestion. The versatility of the click reaction would also make this approach adaptable to multiple imaging modalities, depending on the need. Here we report a proof of concept study that satisfies the criteria stated above. The click-able functional group was introduced by virtue of an orthogonal translation system (OTS) that enables the probiotic Escherichia coli Nissle 1917 (EcN) to incorporate the NSAA p-azido-phenylalanine (pAzF) at UAG (amber) stop codons.24 The strain also harbors a gene expressing an extracellularly displayed protein, csgA, containing an in-frame UAG codon mutation. Together, these modifications enable the bacteria to incorporate and display the bioorthogonal chemical handle during residence in the GI tract that can be targeted by a click-able imaging probe of choice (Figure 1).

tissue biopsies in larger animals, or can be performed at the end points of small animal studies, which hinders longitudinal studies and real-time tracking. Therefore, less invasive tools to track the spatiotemporal dynamics of gut microbes in vivo would be useful for microbiome study. The need for such tools is further underscored by recent efforts to use living microbes as orally deliverable therapeutics and diagnostics.11−16 Unlike traditional drugs, whose pharmacokinetics and pharmacodynamics (PK/PD) can be tracked experimentally with medical imaging techniques, or predicted based on well-established models, microbial PK/PD is comparatively harder to characterize. Indeed, microbes exhibit a range of context-dependent active processes, including selfreplication, chemotaxis, and biochemical communication with other cells in their environment, that make it difficult to determine their biodistribution in a time-resolved manner. Thus, if living microbes are to be treated as sophisticated versions of drugs or drug delivery vehicles, we must develop better tools to track their trafficking and interactions with their surroundings using medically relevant imaging techniques. There are some techniques to track labeled microbes in vivo. One common method involves genetically engineering microbes to express luciferase or fluorescent proteins so that they can be imaged using in vivo imaging techniques.17−19 However, the poor tissue permeability of optical wavelengths limits the use of such techniques to small animals. Additionally, since most of the GI tract is anaerobic, low oxygen availability can inhibit the proper function of certain fluorophores and chromophores and limit the signal that is produced.20 Furthermore, the spatial resolution of optical imaging on small animals reveals little about the location of the microbes in the gut or in other organs. Another recent example used click chemistry to fluorescently label anaerobic bacteria displaying azido sugars on their surface.21−23 This enabled prelabeled bacteria to be tracked during their transit through the GI tract. However, the technique required metabolic incorporation of azido sugars in the bacteria prior to ingestion, so progeny cells were no longer labeled, precluding the longitudinal tracking of the microbes beyond 24 h. An ideal in vivo tracking system for microbes in humans and other large animals should satisfy two primary criteria. First, the spatial localization of the microbes should be ascertainable with



RESULTS Azide-Containing Proteins Are Successfully Secreted and Assembled Extracellularly from Engineered E. coli Nissle 1917. In order for the incorporated pAzF to be accessible to imaging probes, we reasoned that it had to be displayed extracellularly. We incorporated the requisite in-frame UAG codon into the csgA gene, which encodes for curli fibers. Curli are a biofilm matrix component native to E. coli that are produced through the secretion and self-assembly of the CsgA protein into cell-anchored amyloid fibers.25,26 We created two plasmid constructs, pBbB8k-wt and pBbB8k-mut, that contained either the wild-type (wt) or mutant csgA (mut csgA), respectively, in the same cistron as the other curli genes necessary for secretion and assembly, all under the control of an inducible promoter (PBAD). The mut csgA was generated in such a way that the UCA codon that normally encodes for serine at position 89 in the CsgA amino acid sequence was mutated to an amber stop codon (UAG) (Figure S1), which can be recognized by the OTS to incorporate the pAzF in this location during translation. S89 was chosen for the location of 1641

DOI: 10.1021/acssynbio.8b00135 ACS Synth. Biol. 2018, 7, 1640−1650

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Figure 2. Engineered bacteria can produce mutant curli fiber. (A) Amyloid production assay for various strains, based on Congo Red binding, with and without induction. (B) Whole-cell filtration ELISA assays with anti-HIS antibody detection confirms the presence of extracellular HIS-tagged curli fibers under appropriate conditions. Ordinary one way ANOVA with Tukey’s multiple comparison test n = 3, *P < 0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001. (C) Scanning electron microscopy of PBP8 transformed with various plasmid combinations: (−) no plasmid (1) pBb8k-wt (containing wild-type csgA) (2) pBb8k-wt and pEVOL-pAzF (containing OTS) (3) pBb8k-mut (containing mutant csgA) and pEVOL-pAzF. All samples with curli genes successfully express curli fibers including the mutant curli fibers (scale bar = 1 μm).

Figure 3. In vitro click chemistry-dependent labeling of engineered curli fibers. (A) Fluorescence signal from cell cultures spotted onto nitrocellulose membranes and labeled with Cy5-DBCO. Ordinary one way ANOVA with Tukey’s multiple comparison test n = 3, *P < 0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001. (B) Fluorescence signal after labeling of curli amyloid mats after cell removal. (C) SDS-PAGE analysis of lysed cells after induction and semipurification of curli fibers. Coomassie blue stained gel (left) and fluorescence signal from unstained gel (right). (D) Ratio of labeled CsgA to total labeled proteins from various experiment conditions (E) Fluorescence intensity of CsgA variants as a function of pAzF concentration. 1642

DOI: 10.1021/acssynbio.8b00135 ACS Synth. Biol. 2018, 7, 1640−1650

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Figure 4. Labeling efficiency of engineered bacteria. (A) Flow cytometry histogram of cell cultures under various conditions after exposure to Cy5DBCO. (B) Confocal fluorescent micrographs of PBP8 harboring pBb8k-mut and pEVOL-pAzF after induction and labeling.

strain and those harboring either plasmid with and without induction (Figure S5), suggesting that neither OTS nor curli expression negatively affects growth. Engineered Curli Fibers Containing Nonstandard Amino Acids Can Perform Click Chemistry In Vitro. To determine the ability of the mutant curli fibers to perform click chemistry labeling, we exposed induced broth cultures to a Cy5-dibenzocyclooctyl (DBCO) conjugate, a probe designed to react with pAzF. In this case, the cycloalkyne group of DBCO is able to undergo copper-free click chemistry with the azide moiety of pAzF.36 After exposure to the probe conjugate, the bacterial cells were pelleted and washed by resuspending several times in PBS, then aliquots were spotted onto a nitrocellulose membrane and imaged. As expected, PBP8 cultures induced to express mutant curli gave the highest fluorescence signal. However, induced cultures producing wildtype curli exhibited increased signal over the background, suggesting that nonspecific adsorption of the Cy5 dye to curli fibers could be a factor in determining labeling efficiency (Figure 3A). The click reaction yield was not affected significantly by Cy5-DBCO concentrations above 20 μM and labeling times above 1 h, underscoring the robustness of the azide-DBCO reaction for rapid labeling under a range of conditions (Figure S6). To test the labeling efficiency of the mutant curli fibers while removing the effects of nonspecific binding to the bacterial cells themselves, we performed labeling reactions on crudely purified curli fibers. We employed a previously established isolation protocol to obtain curli fiber mats in the absence of cells.37 The filter membrane-supported curli mats were incubated with Cy5DBCO, washed, and imaged (Figure 3B). The fluorescence results indicate that the dye bound specifically to the curli fiber mats only when the mutant fibers, OTS, and pAzF were present. Click Labeling Is Specific to Mutant Curli Fibers. We selected the OTS designed for pAzF incorporation at UAG sites (pEVOL) for several reasons. First, pAzF and the pEVOL system are well-characterized and have been shown to have high incorporation efficiency into mutant proteins.24,35 Second,

the mutation because the native serine residue is predicted to be surface-accessible in the assembled amyloid state, based on multiple structural models of the parallel β-sheet structure of CsgA.27−29 Hence, we reasoned that the location of the mutation would interfere neither with CsgA’s structure nor its assembly into amyloid fibers. A separate plasmid construct (pEVOL-pAzF) harbored the OTS, encoding for a tRNA and an aminoacyl tRNA synthetase that worked together to incorporate pAzF specifically and orthogonally at UAG codons. All in vitro experiments were performed with an EcN-derived strain called PBP8, harboring chromosomal deletions of all the curli genes (EcN::ΔcsgBACDEFG). The genotype of PBP8 was confirmed by sequencing (Figure S2) and its phenotype was confirmed by decreased staining with the amyloid-specific dye, Congo Red,30,31 compared to the parent EcN strain under conditions known to produce curli fibers (Figure S3).32,33 PBP8 cotransformed with pEVOL-pAzF and either pBbB8kwt or pBbB8k-mut successfully produced amyloid fibers in the presence of inducer and pAzF, as confirmed by a quantitative Congo Red (CR) binding assay. In contrast, when any of the necessary componentsOTS, csgA mut gene, or inducer were omitted, less CR binding was observed (Figure 2A). The identity of the extracellular amyloid was confirmed with a whole-cell filtration ELISA that measured the C-terminal His-6 tag on both wt and mutant CsgA (Figure 2B). Electron microscopy of induced cultures further confirmed the ability of the cotransformed PBP8 to produce amyloid fibers with the same morphological features as wild-type curli fibers (Figure 2C). Notably, induced mutants in the absence of pAzF produced a truncated version of CsgA, which could also assemble into amyloid fibers (Figure S4). However, overproduction of this truncated CsgA could lead to slower growth of the engineered cells, which did not happen when the cells were induced in the presence of pAzF (Figure S5). Overproduction of recombinant proteins can be metabolically taxing, hindering the ability of engineered bacteria to compete in the stringent environment of the gut.34,35 We used growth curves of engineered EcN strains to evaluate fitness. We observed little variation in doubling times between the parent 1643

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Figure 5. Engineered bacteria are labeled via click chemistry in vivo. (A) Fluorescence imaging of live mice fed with either PBS only (−), or PBP8 harboring pBbk8-mut and pEVOL-pAzF (+). The mice were given arabinose and pAzF to induce mutant curli expression 2 days prior to the start of the experiment. Images were taken at a different time points after Cy5-DBCO administration at time = 0 h. (B) Representative fluorescence images of harvested mouse GI tracts, collected 36 h after Cy5-DBCO administration under various conditions: (−) negative control with no bacteria or dye administration, (1) no bacteria, (2) no bacteria, but with pAzF in drinking water, (3) PBP8 expressing wt-csgA, (4) PBP8 expressing wt-csgA with pAzF in water, (5) noninduced PBP8 expressing mut-csgA with OTS, (6) PBP8 expressing mut-csgA with OTS. (C) Quantification of Cy5 fluorescence signals from the lower GI tracts. Ordinary one way ANOVA with Tukey’s multiple comparison test n = 3, *P < 0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001. (D) SDS-PAGE analysis of homogenized cecal contents stained with Coomassie blue (top) and unstained fluorescent imaging (bottom). Lane markers correspond to numbering in part B.

UAG is the rarest codon in the E. coli genome, with only 366 instances in EcN. Notably, efforts have been made to increase the specificity and efficiency of NSAA incorporation by replacing all native instances of UAG with a synonymous stop codon across the E. coli genome, permitting the deletion of release factor-1 (RF-1), which terminates translation at UAG codons.38 Since we did not use a recoded strain for this work, there remained the possibility of pAzF incorporation at other genes terminated by UAG in the presence of the OTS. Although it was unclear how much this would affect the success of the in vivo labeling scheme, we wanted to characterize the level of pAzF incorporation in proteins other than CsgA and demonstrate the preferential binding of the dye to the mutant CsgA. We performed SDS-PAGE analysis on semipurified labeled lysed cells to determine the distribution of dye across the PBP8 proteome (Figure 3C). In the Coomassie-stained gel, the semipurified proteins from cultures expressing wild-type curli with and without the OTS showed stronger CsgA bands near 17 kDa, compared to those expressing mutant CsgA (Figure 3C). This is perhaps the result of inefficient translation of full-length CsgA, since pAzF incorporation must compete with premature termination from the cell’s native RF-1. The fluorescence-imaged gel showed that cells expressing mut csgA

and the OTS exhibited higher intensity for the CsgA band compared to other background proteins in the lysate, whereas those expressing wild-type fibers showed higher nonspecific labeling of other proteins. Expressed as a ratio of fluorescence intensities between (CsgA):(all other proteins), the labeling specificity for CsgA was 45× higher when the mut csgA gene was present compared to the wt csgA gene, in the presence of the OTS (Figure 3D). Even with the lower absolute amount of mutant CsgA, we observed much higher dye labeling efficiency for the mutant CsgA compared to wild-type CsgA. Furthermore, the fluorescence intensity of the CsgA band in the gel increases in a dose-dependent manner with pAzF concentration, with labeling being indistinguishable from background signal at a concentration of 0.05 mM (Figure 3E). Labeling Efficiency of Engineered Bacteria. We assessed the labeling efficiency on a per cell basis by subjecting bacterial cultures that had been induced to produce curli fibers and exposed to Cy5-DBCO to flow cytometry analysis. This confirmed that there was some dye association with cells producing wild-type CsgA both without (17.9% labeling) and with (26.2% labeling) the OTS present. However, more than 63.8% of PBP8 cells producing mutant CsgA in the presence of the OTS and the NSAA were labeled (Figure 4A, Figure S7). 1644

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The nonspecific labeling appeared to be dependent on curli production, since it was present at a lower level in the case of untransformed or noninduced PBP8 cells, corroborating the results shown in Figure 3B. Confocal microscopy qualitatively supported the flow cytometry data, with more than half of the cells exhibiting a signal for the Cy5 dye (Figure 4B). Engineered Probiotic Bacteria with Mutant Curli Fibers Are Able To Perform Click Chemistry In Vivo in Murine Model. In order to demonstrate the feasibility of performing the labeling reaction in vivo, we administered the engineered EcN to mice via oral gavage and induced the expression of mutant curli using arabinose and pAzF in their drinking water. Cy-5-DBCO was administered orally 42 h after administering the bacteria, and Cy5 fluorescence signals from the abdominal area were detected using an in vivo imaging system (IVIS) over the course of 48 h (Figure 5A). Fluorescence intensity remained high in mice that had been administered the engineered PBP8 up to 24 h after dye administration. Control experiments with no bacterial administration showed signal decay after 6 h. However, subsequent experiments with noninduced bacteria made it difficult to distinguish click chemistry-based labeling from nonspecific dye binding and tissue autofluorescence (Figure S8). We, therefore, sought to demonstrate the specificity of the labeling reaction using ex vivo methods and additional experimental conditions (i.e., with and without bacteria administration, dye administration, and pAzF administration). On the basis of the previous experiments, we selected 36 h postdye administration as an experimental end point that would ensure that even nonspecifically bound dye would have been cleared from the GI tract. The in vivo experimental scheme is depicted in Figure S9. After harvesting of the GI tracts, Cy5 signal was measured using the IVIS. Significant tissue/food autofluorescence was observed from the stomach, so analysis was confined to the cecum and lower intestine. Qualitative and quantitative analysis showed that the experimental group containing all the necessary components (bacteria, mutant CsgA, pAzF, and inducer) showed a distinct increase in fluorescence intensity measured at 675 nm in the cecum, which is the primary location of E. coli in the mice,39 compared to any of the other experimental conditions (Figure 5B,C). Low intensities were observed in the cecum of mice that had been administered bacteria producing wild-type curli fibers, which correlated to the nonspecific dye adsorption observed in vitro (Figure 5B, panels 3 and 4). Conditions in which pAzF was administered without the necessary machinery for incorporation exhibited cecal fluorescence intensities that were not significantly higher than that observed for dye administration alone, suggesting that nonspecific incorporation of pAzF by host cells or other microbes using native machinery did not contribute significantly to the signal observed for the desired click labeling. Finally, we performed SDS-PAGE analysis of homogenized cecum tissue in order to determine if the fluorescence signals that we observed from the lower GI tract were actually from the click-labeled CsgA protein (Figure 5D). Coomassie staining revealed protein bands at the expected size for mutant CsgA (14.7 kDa) in group 3 (induced PBP8, wild-type curli) and group 6 (induced PBP8, mutant curli). Fluorescence analysis of the gels before Coomassie staining revealed that the observed signal could be attributed to these same bands, with higher intensities for the mutant curli. No other labeled proteins were observed, confirming the reaction specificity for the incorporated pAzF probe and engineered bacteria.

Research Article

DISCUSSION

Most existing methods for studying the spatiotemporal dynamics within the gut microbiome rely on analytical techniques that are either indirect (e.g., fecal bioinformatics), or highly invasive (e.g., histology). Less invasive methods to track microbes in live animals would benefit fundamental microbiome research as well as the development of living microbial therapeutics and diagnostics. Here we describe a new method to label engineered bacteria in vivo using bioorthogonal click chemistry. This technique enables monitoring of microbial localization several days after ingestion and should be compatible with any “click-able” imaging probe. This work shows a basic proof-of-concept that such a labeling strategy can be successfully performed. However, there are several ways in which the technique could be improved upon. The in vitro results suggest that inefficient translation of the mutant CsgA, even in the presence of the OTS, could limit the amount of CsgA that was produced. Although we did not find this to prevent the proof-of-concept demonstration, a recoded E. coli strain might significantly improve the NSAA incorporation efficiency by removing the possibility for premature termination via RF-1. The labeling efficiency on a per microbe basis in vitro was also only ∼60%, which we speculate was related to the well-documented nature of arabinose-inducible promoter systems.40 This suggests that further optimization of promoter systems could also contribute to higher signals in vivo. Detachment of curli fibers from bacteria in the gut could also complicate interpretation of the imaging results, so other proteins bound directly to the cell surface could be worth exploring as alternative labeling targets. Other cell-surface proteins as labeling targets could also ameliorate the nonspecific dye labeling observed for assembled CgsA. Autofluorescence of the upper GI tract and long clearance times for the Cy5-DBCO dye also hindered effective in vivo imaging of the engineered bacteria. Other imaging probes with further red-shifted emissions or probes that incorporate a “turn-on” function upon undergoing the click reaction could improve signal-to-noise ratios. With regard to the potential toxicity of pAzF as in vivo, there is limited data. It is worth noting that copper-free chemistry using Cy5-DBCO has been performed in live mice and rat with no apparent toxicity.41−44 We did not observe any apparent toxicity in our short-term study, though a more thorough toxicity study may have to be performed in the future to assess the safety of pAzF in mouse models. The approach we demonstrate here could enable the development of analytical techniques with new capabilities. For example, the in-frame UAG mutation could be used to report specifically on the production of other extracellularly displayed proteins. Furthermore, the proliferation of OTS systems compatible with different NSAAs and organisms could enable a multiplexed approach to tracking multiple microbes simultaneously. By changing the nature of the probe, one could envision longitudinal, noninvasive imaging of microbial populations in humans or large animals using clinical imaging modalities, like MRI or PET, which enhance tissue penetration in the way that fluorescence or luminescence signals cannot. Excitement for such prospects must be tempered with the requirement that the cellular population to be tracked using this technique must be genetically engineered to enable NSAA incorporation. However, with the meteoric rise of CRISPR/ Cas9-based techniques to rapidly modify genomes and the 1645

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Colonies that are resistant to chloramphenicol were selected and verify the curli operon knockout by colony PCR and genomic DNA sequencing comparing to wild-type EcN. Mice. Female 6- to 8-week-old C57BL/6 mice were purchased from Charles River Laboratories. Mice were housed in SPF conditions with sterile food and water ad libitum. The animal chow included LabDiets 5K67 and the nonfluorescent food LabDiets 5V5R. Mice were maintained in sterile vinyl isolators equipped with food, water and bedding in the Harvard Medical School animal facility. Before any experiment, mice had at least 1 week to acclimatize to the facility environment. All experiments were conducted in accordance with US National Institutes of Health guidelines and approved by the Harvard Medical Area Standing Committee on Animals. In Vitro Expression of Curli Fibers. PBP8 cells transformed with a pBbB8k plasmid were streaked onto LB agar plates containing 50 μg/mL kanamycin (Teknova). PBP8 cells transformed both with a pBbB8k plasmid and with the OTS plasmid were streaked onto LB agar plates containing both 50 μg/mL kanamycin and 50 μg/mL spectinomycin (RPI). Colonies were picked from the plates and 5 mL cultures were inoculated (in LB containing the appropriate antibiotics). Cultures were grown overnight at 37 °C. The overnight cultures were diluted 100-fold in fresh LB medium containing the appropriate antibiotics, and cultured at 37 °C until they reached an optical density (OD) at 600 nm of 0.6 to 0.8. Arabinose was added to the bacterial cultures at a final concentration of 0.05% to induce protein expression. If NSAA incorporation was desired, the NSAA p-azido-L-phenylalanine (pAzF) (Toronto Research Chemicals) was also added to the cultures to a final concentration ranging between 1 mM and 5 mM. Higher concentrations affected cell growth. Protein expression was allowed to occur at 37 °C overnight. Quantitative Congo Red Binding Assay. The quantitative CR binding assay was adapted from a previously published protocol.32 In brief, one mL of testing bacteria culture was centrifuged at 8000 rpm for 10 min. The pellet was resuspended gently in 0.025 mM CR in phosphate buffered saline (PBS), incubated at 25 °C for 10 min and centrifuged at 15 000 rpm for 10 min. 150 μL of the supernatant was transferred to a 96-well plate with clear bottom (Corning) and the absorbance at 490 nm was read using a BioTek H1 microplate reader. The amount of CR binding was calculated by subtracting the measured absorbance from the 0.025 mM CR in PBS control absorbance and normalized by the OD600 of the culture. Whole-Cell Filtration ELISA. The whole-cell filtration ELISA assay was adapted from a previously published protocol.47,48 In brief, the testing bacteria cultures were chilled on ice for at least 20 min and diluted to OD600 of 0.3 using trisbuffered saline (TBS) (Thermo Fisher Scientific). 200 μL of the diluted samples were added to a Multiscreen-GV 96-well filter plate (0.22 μm pore size; EMD Millipore) and filtered. The sample wells were washed three times with a wash buffer (TBS, 0.1% Tween-20 (Sigma)) and blocked by incubating with 1% bovine serum albumin (BSA) (Sigma) and 0.01% H2O2 (Sigma) in wash buffer for 1.5 h at 37 °C. The 3-time wash step was repeated. The wells were incubated with 50 μL of anti-HIS antibody-horseradish peroxidase (HRP) conjugated (1:200 dilution) (Thermo Fisher Scientific) for 2 h at 25 °C and washed 3 times. 100 μL of Ultra-TMB (3,3′,5,5′tetramethylbenzidine) ELISA substrate (Thermo Fisher Scientific) was added to each well and incubated for 20 min

continuing development of new OTS, this could become increasingly accessible in the near future. Ongoing studies in our lab are focused on the development of a second generation system that, in addition to addressing the issues raised above, would rely on incorporation of the OTS and mutant genes in to the bacterial chromosome so that antibiotic selection would not be required during in vivo deployment. Overall, our approach enables a wider selection of imaging probes compared to conventional microbe tracking methods, such as fluorescent labeling or luminescent proteins expression. Nonprotein dyes or inorganic probes can be utilized because they are provided externally and do not have to rely on oxygen-dependent maturation chemistry, like some fluorescent proteins. Alternatively, the incorporation and display of the azide bearing amino acid could be tied to other environmental sensing mechanisms relevant to the gut,11,45 leading to diagnostics that would report on disease states with spatial resolution within the GI tract. Furthermore, the approach may be useful for tracking the progression of infections in model systems.



EXPERIMENTAL PROCEDURES Cell Strains and Plasmids. The divergent curli operon regions consisting of csgBAC and csgEFG were PCR isolated from E. coli K12 substr. W3110 and cloned by overlap extension into the pBbB8k plasmid, to create a single operon, csgBACEFG, under the control of the araBAD promoter. The cloning of the curli operon was performed in an analogous manner to our previously published work.37 A six-histidine tag (HisTag) was added to the C-terminus of CsgA to allow for immunodetection (pBbB8k-wt) (see plasmid map in Figure S10). A control plasmid was constructed by cloning the malE gene encoding for the maltose binding protein (MBP) from the W3110 genome into the pBbB8k plasmid under the control of the araBp promoter (pBbB8k-MBP). To allow for the incorporation of the NSAA, a mutation encoding for the amber stop codon (UAG) was inserted within the open-reading frame of CsgA (pBbB8k-mut csgA). Using site-directed mutagenesis, we directed the amber mutation in place of a UCA codon, which normally encodes for serine at amino acid position 89 of CsgA (see DNA sequences in Supporting Information 1 and 2). The orthogonal translation system (OTS) plasmid pEVOLpAzF24 was obtained from the Church Lab with slight modification where the chloramphenicol resistance was swapped to spectinomycin resistance and the sequences were codon optimized. Protein expression was performed in a curli operon deletion mutant, PBP8, an E. coli strain derived from Nissle 1917 (EcN). PBP8 strain was constructed using lambda red recombineering method described previously by Datsenko and Wanner.46 In brief, the chloramphenicol acetyltransferase (CAT) cassette was constructed with 500 bp homology arms upstream and downstream of the curli operon using SOEing PCR. The CAT cassette was transformed into electrocompetent EcN with preinduced lambda red genes from the pKD46 plasmid using 0.5% arabinose (Sigma) during the growth step of electrocompetent cell preparation. The transformant was expanded using SOC media at 30 °C shaking incubator for 3 h to promote the genomic replacement of the curli operon with CAT cassette. The transformant was then plated onto lysogeny broth (LB) agar plates (Sigma) containing 25 μg/mL chloramphenicol (RPI) and incubated overnight at 37 °C. 1646

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ACS Synthetic Biology at 25 °C. Then, 50 μL of 2 M H2SO4 (Alfa Aesar) was added to the wells to stop the reaction. 100 μL of this reaction was transferred to a 96-well plate where the absorbance at 450 and 650 nm was measure. The relative amount of displayed HIS tag was obtained by subtracting absorbance at 450 nm with absorbance at 650 nm. Electron Microscopy. Cells expressing curli fibers (with and without pAzF) were imaged by scanning electron microscopy (SEM) to assess the formation of fibers. 100 μL of cell cultures were filtered onto Nucleopore filter membranes (0.22 um pore size, GE Healthcare Bio-Sciences) under vacuum. The samples were fixed with 2% (m/v) glutaraldehyde and 2% (m/v) paraformaldehyde in 0.1 M sodium cacodylate buffer for 2 h at room temperature. The membranes were then gently washed with water, and the solvent was gradually exchanged to ethanol with an increasing ethanol 15 min incubation step gradient (25%, 50%, 75% and 100% (v/v) ethanol). The samples were dried in a critical point dryer, placed onto SEM sample holders using silver adhesive (Electron Microscopy Sciences), and sputtered until they were coated in a 5 nm layer of Pt/Pd. Imaging was performed using a Zeiss Ultra 55 Field Emission SEM. Growth Curves and Doubling Times. The cells were grown in LB broth containing appropriate antibiotics overnight, diluted 1:100 in fresh LB Broth with antibiotics, and grown in a 1 mL 96 well plate at 37°C and shaken at 900 rpm. Once the cells reached an OD600 of 0.6, they were again diluted 1:100 in fresh LB Broth in a 250 mL 96 well plate. Half the cells were induced with 0.05% Arabinose and incubated with 5 mM pAzF. The other half of the cells were used as negative controls and were not induced with Arabinose and were not exposed to pAzF. Cells expressing the curli operon, or, as controls, PBP8 cells, were used. After this preparation, the 96 well plate was placed in a Biotek Kinetics Machine, which measured OD600 every 5 min and shook the plate on medium speed for 24 h. The data were then plotted and the linear slope during exponential growth was used to calculate doubling times. Because curli-expression cells derivatives had more irregular exponential growths than control cells, we used the first exponential growth “hump” of curli variants to determine doubling times. In Vitro Labeling of Click Microbes. Cells expressing curli fibers were pelleted at 4000g for 10 min. The cells were resuspended in phosphate buffer saline (PBS) containing 1% (m/v) bovine serum albumin (BSA). The centrifugation and resuspension process was repeated 3 times to clean the cells from any excess free NSAA present in the culture medium. The appropriate volume for the experiments was taken (200 μL of OD 5 per sample), pelleted and incubated at OD600 of 10 in 100 μL Cy5-DBCO (5 μM) in PBS + 1% BSA for 2 h at 37 °C with agitation. The labeled cells were pelleted again and resuspended in PBS containing 3% (m/v) BSA. This washing step was repeated 3 times to remove unbound dye. Labeling was assessed by spotting 10 μL of labeled cells on a nitrocellulose membrane and detecting the fluorescence of Cy5 using a FluorChem M system (Protein Simple). Labeling of Simulated Curli Fiber Mats. Curli fiber mats from bacteria in different conditions were created by following published protocol.37 In brief, we used E. coli PQN4 lab strain, which has been previously characterized to produce a high amount of curli materials.37 Following curli expression protocol, we induced PQN4 wild type curli, wild type curli with OTS and mutant curli with OTS by adding 0.05% arabinose and 0.1 mM

pAzF in the culture media. After the induction period, guanidinum chloride (GdmCl) (Sigma) was added to the cultures to 0.8 M final concentration and incubated for 1−2 h at 4 °C prior to filtration. 30−50 mL of the GdmCl treated cultures were vacuum-filtered onto polycarbonate filter membranes (47 mm diameter, 10 μm pore size, EMD Millipore). The filter membranes were incubated with 5 mL of 8 M GdmCl for 5 min and vacuum filtered to eliminate the cell debris, and rinsed with 5 mL of deionized water 3 times. Then, the membranes were incubated with 5 mL of nuclease solution (1.5 U/mL of Benzonase, EMD Millipore, with 2 mM MgCl2 (Sigma)) for 10 min and vacuum filtered to remove remaining nucleic acids, and rinsed with 5 mL of deionized water 3 times. Then, the semipurified curli fiber mats on the filters were incubated with 2 mL 5 μM Cy5-DBCO for 1 h and rinsed with 5 mL of deionized water 3 times to remove unbound dyes, before imaging with a FluorChem M system (Protein Simple). Purification and Identification of Proteins Labeled In Vitro. 500 mL of prelabeled cells at OD600 1 were pelleted at 4000g for 20 min and resuspended in 30 mL of lysis buffer (50 mM phosphate buffer, 300 mM NaCl, 7 M guanidinium hydrochloride). A protease inhibitor cocktail was added, and the suspension was stored at −20 °C overnight. The suspension was thawed on ice and sonicated to fully lyse the cells (40% amplitude, 3 × 25s ON, 35s OFF, QSONICA Q700 Sonicator). After centrifugation at 10 000g for 30 min, the supernatant was applied to a NiNTA beads and incubated 2 h with agitation at room temperature in the presence of 10 mM imidazole. The beads were then transferred into the plastic columns. His-tag purification was performed by washing the column 3 times with 40 mM imidazole, and eluting his-tagged CsgA proteins with 500 mM imidazole (both in 50 mM phosphate buffer with 100 mM NaCl). The eluate was concentrated using 3 kDa Amicon ultracentrifugal filters (EMD Millipore) and ran on a 4−20% SDSPAGE gel. Prior to staining with Coomassie blue, the Cy5 fluorescence within the gel was detected. Flow Cytometry and Confocal Microscopy. Flow cytometry was used to determine the fraction of cells that were labeled. The cells were further diluted to an OD600 of 0.01 per mL in PBS and analyzed with a BD LSRFortessa Flow Cytometer System (BD Biosciences) using the APC channel for Cy5 fluorescence detection. For confocal microscopy the cells were also stained with 5 μM Hoechst 33342 (Thermo Fischer Scientific) in 1× PBS for 1 h and washed 3 times with 1 mL of PBS. Subsequently, the cells were fixed in 2% paraformaldehyde for 10 min at 25 °C and washed 3 times with 1 mL of PBS. Ten μL of cells were deposited on a glass slide for imaging with a Leica SP5 X MP Inverted Confocal Microscope (Leica Microsystems). In Vivo Tracking of Click Microbes. Prior to the experiment, mice were given a nonfluorescent food (alfalfafree) for at least 5 days to minimize background autofluorescence. At 12 h prior to oral gavage of bacteria, mice were fasted and given special water containing antibiotics (1 g/L kanamycin, 1 g/L spectinomycin), inducer (10 g/L L(+)-arabinose) and pAzF (5 mM) based on their assigned experimental conditions. The inducer concentration was chosen based on comparison to previously published examples of engineered bacteria in mice.16,49 Then, the starting culture of PBP8 transformed with pBbB8k-wt was expanded 1:100 dilution in LB containing 50 μg/mL kanamycin, while that of 1647

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FluorChem M system (Protein Simple). Then, the gels were stained with Coomassie Brilliant Blue to detect the presence of proteins and compared the size against standard protein ladder (Bio-Rad).

PBP8 transformed with pBbB8k-mut and pEVOL-pAzF was expanded 1:100 dilution in LB containing 50 μg/mL kanamycin and spectinomycin to OD600 of 0.5. The log-phase cultures were centrifuged at 4000 g for 15 min at 4 °C and resuspended in 20% sucrose (OmniPur) in PBS to OD600 of 10. Once the mice have been fasted for 12 h, 100 μL of the prepared log-phase bacteria were administered to the mice via oral gavage. The alfalfa-free food was returned to the mice as well as the special water to allow proliferation and protein induction of engineered bacteria inside the mouse gut. Meanwhile, the mouse’s abdominal hair was removed to allow the upcoming IVIS imaging. Thirty hours after the bacteria gavage, mice were fasted for another 12 h to remove the food from the GI tract. 10 h after that, the NSAA and arabinose containing water was switched into antibiotic-only water to prepare the mice for dye administration. Two hours after the water has been switched and the food has been withheld, 100 μL of 100 μM of Cy5-DBCO in 20% sucrose in PBS are administered to the mice by oral gavage. The alfalfa-free food and antibiotic water were returned to the mice. Then, mice were imaged under anesthesia using IVIS Lumina II (PerkinElmer) at t = 0 (before the gavage), 6, 11, 24, and 48 h. The IVIS instrument is equipped with 10 narrowband excitation filters (30 nm bandwidth) and 4 broadband emission filters (60 and 75 nm bandwidth). At time point, the mice were imaged using excitation filter at 675 nm, and 500 nm for background subtraction, and emission filter at 695−770 nm, with field of view (FOV) = D (12.5 cm), fstop = 2 and medium binning. Living Image software version 4.3.1/4.4 was used for image analysis. Whole GI Tract Ex Vivo Fluorescence Imaging. The mouse experiment was performed in the same manner as the in vivo tracking experiment up to the dye administration. 36 h following the dye administration, the mice were euthanized to harvest the whole GI tract for ex vivo fluorescence imaging. The GI tract was placed on the lid of 150 × 25 mm polystyrene tissue culture plate (Falcon) and imaged using IVIS Lumina II with the same setting as the in vivo imaging. After imaging, the GI tract was kept at −20 °C for protein extraction. The images were then analyzed using ImageJ software for the fluorescence signal from the lower GI tract. Whole Cecum Fluorescence and Protein Analysis. The GI tract specimens used in the ex vivo fluorescence imaging were further analyzed for curli and Cy5-DBCO interaction. The mouse GI tracts were removed from −20 °C. The cecum from each sample was excised, transferred to a 15 mL falcon tube, and crushed to homogenize. Three mL of PBS was added to each sample, supplemented with 4 μL of benzonase nuclease (Novagen) and 8 μL of 1 M magnesium sulfate (MgSO4) (Sigma). The samples were incubated at 37 °C overnight. Each sample was transferred to 2 mL microtube and centrifuged at 14 000 rpm for 10 min to extract the supernatant. The supernatant samples were transferred to another set of tubes, and concentrated using 10-kDa Amicon Ultra 0.5 mL centrifugal filters (Millipore) at 10 000 rpm centrifugation for 15 min twice. The pellet samples were resuspended in 200 μL of PBS. Both supernatant and pellet samples were diluted five times, mixed with 2× dyeless Laemli buffer in 1:1 ratio, incubated at 95 °C for 5 min and run on 12% SDS-PAGE gel (Bio-Rad) at 200 V for 30 min. After the gel electrophoresis, the gels were rinsed with water and imaged to detect the fluorescence of Cy5 using a



ASSOCIATED CONTENT

S Supporting Information *

The Supporting Information is available free of charge on the ACS Publications website at DOI: 10.1021/acssynbio.8b00135. Figures S1−S10, csgA sequences (PDF)



AUTHOR INFORMATION

Corresponding Author

*E-mail: [email protected]. ORCID

Neel S. Joshi: 0000-0001-8236-3566 Author Contributions ■

P. Praveschotinunt and N.-M. Dorval Courchesne contributed equally. P.P., N.-M.D.C., and N.S.J. conceived the idea and designed the experiments. P.P., N.-M.D.C., and J.J.K. performed the curli characterization experiments and data analysis. N.-M.D.C., I.D.H., C.L., and J.J.K. performed the in vitro labeling experiments and data analysis. P.P., I.D.H., and C.L. performed the in vivo experiments and data analysis. P.P. performed the curli operon knockout in the PBP8 strain. P.Q.N. cloned the wt csgA plasmid. N.-M.D.C. cloned the mut csgA plasmid. J.J.K. performed the growth curve experiments and analysis. The manuscript was written with contributions from all authors and all authors approve the manuscript.

Author Contributions □

I. den Hartog and C. Lu contributed equally.

Notes

The authors declare no competing financial interest.



ACKNOWLEDGMENTS This work made use of the Harvard Center for Nanoscale Systems (CNS) and Harvard Medical School ICCB-Longwood Screening Facility, and the Wyss Institute for Biologically Inspired Engineering. We would like to thank Alexis Rovner, Amanda Graveline, Andyna Vernet, Frank Urena, Thomas Ferrante, Garry Cuneo and Franziska Bahl for their help. P.P. thankfully acknowledges the royal Thai government scholarship. N.-M.D.C. gratefully acknowledges a Postdoctoral research fellowship from the Fonds de Recherche Nature et Technologies du Québec (FRQNT). J.J.K thankfully acknowledges the Harvard College Program for Research in Science and Engineering (PRISE) and the Harvard College Research Program (HCRP) fellowships. This work was supported by National Institutes of Health (1R01DK110770-01A1) and the Wyss Institute for Biologically Inspired Engineering.



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